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Isolation and Characterization of o-Xylene Oxygenase Genes from Rhodococcus opacus TKN14

机译:不透明红球菌TKN14的邻二甲苯加氧酶基因的分离与鉴定

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摘要

o-Xylene is one of the most difficult-to-degrade environmental pollutants. We report here Rhodococcus genes mediating oxygenation in the first step of o-xylene degradation. Rhodococcus opacus TKN14, isolated from soil contaminated with o-xylene, was able to utilize o-xylene as the sole carbon source and to metabolize it to o-methylbenzoic acid. A cosmid library from the genome of this strain was constructed in Escherichia coli. A bioconversion analysis revealed that a cosmid clone incorporating a 15-kb NotI fragment had the ability to convert o-xylene into o-methylbenzyl alcohol. The sequence analysis of this 15-kb region indicated the presence of a gene cluster significantly homologous to the naphthalene-inducible dioxygenase gene clusters (nidABCD) that had been isolated from Rhodococcus sp. strain I24. Complementation studies, using E. coli expressing various combinations of individual open reading frames, revealed that a gene (named nidE) for rubredoxin (Rd) and a novel gene (named nidF) encoding an auxiliary protein, which had no overall homology with any other proteins, were indispensable for the methyl oxidation reaction of o-xylene, in addition to the dioxygenase iron-sulfur protein genes (nidAB). Regardless of the presence of NidF, the enzyme composed of NidABE was found to function as a typical naphthalene dioxygenase for converting naphthalene and various (di)methylnaphthalenes into their corresponding cis-dihydrodiols. All the nidABEF genes were transcriptionally induced in R. opacus TKN14 by the addition of o-xylene to a mineral salt medium. It is very likely that these genes are involved in the degradation pathways of a wide range of aromatic hydrocarbons by Rhodococcus species as the first key enzyme.
机译:邻二甲苯是最难降解的环境污染物之一。我们在这里报告了在邻二甲苯降解的第一步中介导氧合的红球菌基因。从被邻二甲苯污染的土壤中分离出的不透明红球菌TKN14,能够利用邻二甲苯作为唯一的碳源并将其代谢为邻甲基苯甲酸。在大肠杆菌中构建了该菌株基因组的粘粒文库。生物转化分析表明,掺入15kb NotI片段的粘粒克隆具有将邻二甲苯转化为邻甲基苄醇的能力。该15kb区域的序列分析表明存在与从红球菌属sp中分离出的萘可诱导的双加氧酶基因簇(nidABCD)显着同源的基因簇。 I24株。使用表达个别开放阅读框的各种组合的大肠杆菌进行的补充研究表明,一个红霉素(Rd)的基因(名为nidE)和一个编码辅助蛋白的新基因(名为nidF)与其他蛋白质没有总体同源性除双加氧酶铁硫蛋白基因( nidAB )外,蛋白对于邻二甲苯的甲基氧化反应也是必不可少的。无论NidF的存在如何,都发现由NidABE组成的酶起典型的萘双加氧酶的作用,将萘和各种(di)甲基萘转化为相应的顺式-二氢二醇。所有 nidABEF 基因均在 R中转录诱导。通过向矿物盐介质中添加 o -二甲苯来制备TKN14。这些基因很可能参与了红球菌作为第一关键酶的多种芳香烃的降解途径。

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